Viral Zoonoses in Small Wild Mammals and Detection of Hantavirus, Spain

We screened 526 wild small mammals for zoonotic viruses in northwest Spain and found hantavirus in common voles (Microtus arvalis) (1.5%) and high prevalence (48%) of orthopoxvirus among western Mediterranean mice (Mus spretus). We also detected arenavirus among small mammals. These findings suggest novel risks for viral transmission in the region.

W ildlife viromes harbor potentially threatening zoonoses for humans that require increased effort in identification and surveillance (1). Rodents are considered main reservoirs of emerging zoonoses (2), and the large population fluctuations of reservoir species play a key role in modulating infection risk (3). Anthropogenic land-use changes, agricultural intensification, and irrigation also favor rodent invasions and risk for pathogen spillover (4). The common vole (Microtus arvalis) is a widespread rodent inhabiting intensified farming landscapes in northwestern Spain, where population numbers and pathogen prevalence lead to spillover of zoonotic bacteria such as Francisella tularensis and Bartonella spp. (5).
We report the prevalence of rodent-borne zoonotic viruses in Europe (i.e., hantavirus, arenavirus [lymphocytic choriomeningitis virus (LCMV)], and orthopoxvirus) (6) among the small mammals inhabiting farming landscapes. We also report the effect of natural fluctuations of common vole numbers on viral prevalence (phase dependence). Our study was conducted in intensively farmed landscapes, in the Tierra de Campos region of Castillay-León, northwestern Spain (7), where the small mammal population is mainly composed of 4 species: common vole, long-tailed field mouse (Apodemus sylvaticus), western Mediterranean mouse (Mus spretus), and greater white-toothed shrew (Crocidura russula) (7).
We live-trapped small mammals during March 2013-March 2019. We collected samples from blood, spleen, liver, and lungs by using standard protocols and stored them at -23°C until molecular analysis could be performed (Appendix, https://wwwnc. cdc.gov/EID/article/28/6/21-2508-App1.pdf). We owned all necessary licenses and permits for conducting this study.
We detected specific hantavirus, LCMV, and orthopoxvirus IgG in serum samples by using immunofluorescence assay. We used fluorescein isothiocyanate (FITC) anti-IgG as a secondary antibody and evaluated all slides under a fluorescence microscope. For molecular analysis, we isolated RNA from liver and lung tissues and DNA from a mix of liver and spleen. We performed single-step reverse transcription PCR (RT-PCR) for LCMV detection in the liver, nested reverse transcription PCR for hantavirus detection in lung samples, and conventional pan-poxvirus PCR method followed by an additional orthopoxvirus-specific PCR for orthopoxvirus detection in the mix samples. We used generalized linear models to test variations of prevalence between species and calculate prevalence in common voles according to host sex (male or female), trapping month (March, July, or November), and population density phase (increase, peak, or crash).
We screened 526 individual animals from 4 species for the presence of 3 viruses (Table; Appendix). We found evidence of hantavirus infection only in

RESEARCH LETTERS
We screened 526 wild small mammals for zoonotic viruses in northwest Spain and found hantavirus in common voles (Microtus arvalis) (1.5%) and high prevalence (48%) of orthopoxvirus among western Mediterranean mice (Mus spretus). We also detected arenavirus among small mammals. These findings suggest novel risks for viral transmission in the region.
Recent surveys of viral zoonoses in Spain have shown low antibody prevalence of LCMV (1.7%) (8) and hantavirus (0.06%) (9) among humans. Hantavirus antibodies were detected in red foxes (Vulpes vulpes) (10), and LCMV antibodies were detected in long-tailed field mice and red foxes (8,10). Our study detected hantavirus in a wild rodent reservoir in Spain. The reported prevalence was low (1.6%) and did not differ between the phases of the common vole population cycle. However, the cyclic dynamic of this rodent host, which harbored all 3 virus species screened, may influence the risks associated with contact with infected rodents. Common voles can reach densities of up to 1,000 per hectare during population peaks, so the infected proportion may become a considerable public health concern. Orthopoxvirus infection risk is of growing concern in Europe because of the absence of smallpox vaccination among the human population <45 years of age (6). Because half of all the western Mediterranean mice analyzed were positive for orthopoxvirus, the potential transmission risk for the virus from this rodent to humans should be considered and further confirmed with larger sample sizes.
Further investigation is required regarding the molecular nature and infectivity of the hantavirus and orthopoxvirus detected, as well as their circulation pathways, which will help to uncover possible transmission routes and determine more precisely the level of infection risk to human populations. Our results can be used by local authorities to refine virus surveillance, including clinical diagnosis of new viruses, and improve public health strategies to prevent and minimize zoonotic risks for persons living in areas recurrently affected by outbreaks linked to common voles. T o limit spread of novel SARS-CoV-2 variants such as Omicron B.1.1.529, early detection is crucial. Wastewater surveillance has been suggested as an early warning system for SARS-CoV-2 spread in lowprevalence areas or communities where human testing is limited (1).

RESEARCH LETTERS
We provide a method to rapidly determine the presence of Omicron in wastewater samples that have low viral load, in which the Omicron genome

RESEARCH LETTERS
We report wastewater surveillance for SARS-CoV-2 variants of concern by using mutation-specific, real-time PCR and rapid nanopore sequencing. This surveillance might be useful for an early warning in a scenario in which a new variant is emerging, even in areas that have low virus incidences.